Question

Normalizing For Batch Effect In RNA-Seq Data

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10.0 years ago

Tom A ▴ 110

Hello,

Does anyone have a suggestion for dealing with "batch effect" between two batches of small RNA-Seq data? I've heard "ComBat" was good. Anyone have any others in mind?

Thanks in advance.

RNA-Seq combat principle-component batch-effect • 6.2k views

ADD COMMENT • link updated 2.6 years ago by Ram 43k • written 10.0 years ago by Tom A ▴ 110

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This paper is worth a look. They tried several methods on array data (including "small" sample sizes), and concluded ComBat performed best: http://www.plosone.org/article/info%3Adoi%2F10.1371%2Fjournal.pone.0017238

ADD REPLY • link updated 4.3 years ago by Ram 43k • written 10.0 years ago by Ahill ★ 1.9k

Ram · Answer 1 · 2014-04-24

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10.0 years ago

Ann ★ 2.4k

The EdgeR package in Bioconductor can help with this. See the Arabidopsis data set in the User's Guide where samples were collected at different times.

ADD COMMENT • link updated 4.3 years ago by Ram 43k • written 10.0 years ago by Ann ★ 2.4k

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Thank you. I will give it a look over.

ADD REPLY • link updated 4.3 years ago by Ram 43k • written 10.0 years ago by Tom A ▴ 110

score 1 · Answer 2 · 2015-11-24

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8.4 years ago

tonja.r ▴ 600

Try RUVseq, they have three different approaches how to deal with batch effects based on empirical genes, in-spike genes and samples contrast. Also, take a look on PEER.

ADD COMMENT • link 8.4 years ago by tonja.r ▴ 600

score 0 · Answer 3 · 2015-11-24

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8.4 years ago

Ron ★ 1.2k

I used combat and it does it pretty well.

ADD COMMENT • link 8.4 years ago by Ron ★ 1.2k